Growth Characteristics and Thermodynamics of Syntrophic Acetate

Apr 16, 2019 - Department of Microbiology, Swedish University of Agricultural ... School of Engineering, Newcastle University, Newcastle-upon-Tyne NE1...
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Energy and the Environment

Growth Characteristics and Thermodynamics of Syntrophic Acetate Oxidizers Maria Westerholm, Jan Dolfing, and Anna Schnurer Environ. Sci. Technol., Just Accepted Manuscript • DOI: 10.1021/acs.est.9b00288 • Publication Date (Web): 16 Apr 2019 Downloaded from http://pubs.acs.org on April 17, 2019

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Growth Characteristics and Thermodynamics of Syntrophic Acetate Oxidizers

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Maria Westerholm1*, Jan Dolfing2, Anna Schnürer1

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1Department

5

750 07 Uppsala, Sweden

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2School

of Microbiology, Swedish University of Agricultural Sciences, Uppsala BioCenter, Box 7025, SE-

of Engineering, Newcastle University, Newcastle-upon-Tyne, NE1 7RU England, UK

7 8 9

*Corresponding

author:

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Maria Westerholm

11

Department of Microbiology, Uppsala BioCenter

12

Swedish University of Agricultural Sciences

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Box 7025

14

SE 750 07 Uppsala

15

Sweden

16

Tel. (+46) 18 671000

17

Fax (+46) 18 673393

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E-mail: [email protected]

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ABSTRACT: Syntrophic acetate oxidation (SAO) plays a pivotal role in biogas production

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processes when aceticlastic methanogens are inhibited. Despite the importance of SAO, the

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metabolic interactions and syntrophic growth of the organisms involved are still poorly

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understood. Therefore we studied growth parameters and interactions within constructed

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defined co-cultures comprising the methanogen Methanoculleus bourgensis and one, or

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several, of the syntrophic acetate oxidizers Syntrophaceticus schinkii, [Clostridium] ultunense,

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Tepidanaerobacter acetatoxydans, and a novel, uncharacterized bacterium. Cultivation

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experiments in a design-of-experiment approach revealed positive effects on methane

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production rate of increased ammonium levels (up to 0.2 M), temperature (up to 45C) and

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acetate concentrations (0.15-0.30 M). Molecular analyses and thermodynamic calculations

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demonstrated close interlinkages between the microorganisms, with available energy of -10

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kJ/mol for acetate oxidation and -20 kJ/mol for hydrogenotrophic methanogenesis. The

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estimated generation time varied between 14-24 days for the bacteria and 13-29 days for the

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methanogen and the acetate minimum threshold level was 0.40-0.45 mM. The rate of

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methanogenesis depended on the SAO bacteria present in the culture. These data are beneficial

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for interpretation of SAO prevalence and competiveness against aceticlastic methanogens in

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anaerobic environments.

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INTRODUCTION

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Anaerobic digestion is an efficient waste management technique to convert organic material to

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biogas, a renewable fuel that can replace fossil fuel in heating/cooling, electrical power

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generation and transportation.1 Several organic wastes from agriculture, households, and food

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manufacturing industries contain proteins, and thus have high biogas potential. The digestate

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generated from these wastes after anaerobic degradation is also a nutrient-rich and valuable

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biofertilizer.2 However, high protein content can be a major drawback in biogas systems, due

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to formation of excess ammonia during protein degradation. Ammonia is toxic to many

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microorganisms and thus often gives rise to process instability and decreased biogas yields.3

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Increasing acetate level is often the first chemical signal of microbial ammonia inhibition, an

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effect related to the reduced activity of ammonia-sensitive aceticlastic methanogens.4 Instead,

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ammonia-tolerant microorganisms performing syntrophic acetate oxidation (SAO) in

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association with hydrogenotrophic methanogens may take over.4, 5 SAO involves a mutualistic

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interaction between syntrophic acetate-oxidizing bacteria and hydrogen (H2)-oxidizing

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methanogens. The syntrophic bacteria oxidize acetate to H2 and carbon dioxide (CO2) or

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formate, which are subsequently converted to methane (CH4) by H2-utilizing methanogens.

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The bacteria rely on the methanogenic activity, since acetate oxidation rapidly becomes

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endergonic when H2 accumulates.6 Nevertheless, the H2 (or formate) level still needs to be

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sufficient to favor the hydrogenotrophic methanogens and is thus restrained within a low and

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narrow range.7

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Only a few bacteria capable of SAO have been isolated and characterized to date. These include

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the mesophiles [Clostridium] ultunense8 and Syntrophaceticus schinkii,9 the thermotolerant

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Tepidanaerobacter acetatoxydans,10 and the thermophiles Thermacetogenium phaeum11 and

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Pseudothermotoga lettingae.12, 13 These bacteria have the special physiological feature that

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they can utilize various substrates in pure culture, in addition to oxidizing acetate in SAO.14

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Co-culturing and genomic studies of some of these isolates have revealed and confirmed

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potential physiological and metabolic capabilities of their syntrophic cooperation.15-20

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However, many key aspects within this area remain unexplored. Thus, further insights into

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syntrophic growth and metabolism are critical in order to reveal the behavior of these

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organisms in response to ecological parameters and their ability to compete for acetate under

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various conditions.

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The aim of the present study was to identify the thermodynamic constraints on SAO under

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mesophilic conditions and to examine the impact of environmental parameters on the growth

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rate of defined SAO co-cultures. The impact of temperature, pH, ammonium, and initial acetate

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concentration on methane production and acetate degradation rate was established in batch

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cultures comprising Methanoculleus bourgensis and one, or several, of the syntrophic acetate

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oxidizers S. schinkii, [C.] ultunense, and T. acetatoxydans and a novel, yet to be characterized,

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bacterium. To allow calculation of thermodynamic constraints, the communities were

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maintained and sub-cultured in medium with sodium acetate as the sole energy source and H2

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partial pressure, pH, temperature, CO2, methane formation, and acetate degradation were

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monitored throughout the growth experiments. The 16S rRNA gene abundance of the main

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species was quantified to obtain information on the interplay between the organisms in the co-

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cultures. The intention was to gain fundamental insights into the syntrophic mechanism of

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acetate oxidation, which will be useful in developing strategies to improve high-ammonia

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biogas processes.

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MATERIALS AND METHODS

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Organisms and Media. The syntrophic acetate-oxidizing bacteria [C.] ultunense strain Esp

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JCM 16670, S. schinkii strain Sp3 JCM 16669,9 and T. acetatoxydans strain T1 DSM 2180410

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and the hydrogenotrophic methanogen M. bourgensis strain MAB121 used in this study were

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isolated at the Department of Microbiology, Swedish University of Agricultural Sciences.

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Recent phylogenetic analysis has affiliated [C.] ultunense to the family Tissierellaceae and not

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Clostridiaceae17. Therefore, the genus name of this species awaits amendment. The family

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name for [C.] ultunense is thus given in brackets. For co-cultivation, S. schinkii and M.

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bourgensis were inoculated (culture cos) and another defined culture was established by

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inoculating all three SAO bacteria and M. bourgensis (culture comix). However, 16S rRNA gene

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Illumina sequencing revealed presence of an additional uncharacterized species, strain AMB1

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(Keratinibaculum paraultunense as closest relative with 96% sequence identity) in the

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methanogenic culture and it was thus also included in the cos and comix cultures.

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All cultures were grown in bicarbonate-buffered basal media with yeast extract (0.2 g/L)

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containing sodium acetate and ammonium chloride (NH4Cl), prepared as described in

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Westerholm et al.9 The initial pH of the media was 7.3. For incubation at pH 8.1, changes in

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medium composition and minor pH adjustments were performed as described in Westerholm

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et al.10 The cultures were grown in serum bottles (Nordic pack, Sweden) sealed with rubber

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stoppers (Rubber Bv, Netherlands) and were inoculated with co-cultures that had depleted

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acetate (100 mM) to below detection. The cultures were incubated in darkness, without

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shaking, at set temperatures. Temperature was monitored continuously during growth.

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Analytical Procedures and Molecular Analyses. Methane and CO2 in the gas phase were

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quantified by gas chromatography and concentration of volatile fatty acids (VFA, including

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acetate, propionate, butyrate, isobutyrate, valeriate, isovaleriate, capronate and isocapronate)

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in the liquid phase was determined using high-performance liquid chromatography as described

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previously.9 In order to determine the final VFA levels, analyses using gas chromatography

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(6890 Series, Hewlett Packard, USA) were conducted as described previously.22 The partial

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pressure of H2 (pH2) was analyzed by direct injection of 1 mL headspace gas (by syringe) from

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the cultures into a gas chromatograph with a reducing compound (HgO bed) photometer (Peak

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Performer Reduced Gas Analyzer PP1, Peak Laboratories, CA, USA). After being separated

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from the matrix gas through a system of two packed columns (a zeolite MS13X 60/80 column

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with length 16.5" and a Unibead silica 1S 60/80 column with length 81") using N2 carrier gas,

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H2 was indirectly detected and quantified by the mercury vapor liberated from the heated HgO

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bed with an ultraviolet (UV, 254 nm) absorption photometer. A dilution of 20 000 ppm H2

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standard (Aga, Sweden) was used for calibration.

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Extraction of total genomic DNA, construction of standard curves, and quantitative polymerase

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chain reaction (qPCR) analysis were conducted as described elsewhere.23 16S rRNA genes of

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[C.] ultunense, S. schinkii, T. acetatoxydans, and M. bourgensis were targeted using primer

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pairs Cult, THAC, Tp, and MAB developed by Westerholm et al.23, 24 For targeting the novel

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strain

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AACGAGCGCAACCCCTATTT-3´)

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CTGGGATCGGCTTTTTGGGA-3´) were designed using Geneious v6.1. To evaluate their

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specificity, these new primers were tested with genomic DNA from pure culture of all strains

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present in the comix culture. The qPCR protocol for analysis of AMB1 consisted of 7 min at

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95°C, 40 cycles of 95°C for 30 s, annealing at 60°C for 1 min and 72°C for 30 s, and finally

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temperature melt curve analysis. Construction of 16S rRNA gene amplicon libraries, Illumina

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MiSeq sequencing, and data analyses were carried out as described previously25, with the

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exceptions that fastp v. 0.19.526 was used for quality control and read filtering, the software

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package Divisive Amplicon Denoising Algorithm 2 (DADA2)27 version 1.6.0 was used for

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further processing, and the forward and reverse reads were truncated at positions 250 and 200,

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respectively. Assignment of taxonomy was performed with the DADA2 taxonomy

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classification, using the Silva training set v. 132. The data were organized into a single data

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object (phyloseq package28) and the graphic was produced using the plot_bar function (ggplot2

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package29) in R Studio software.30 Reads were assigned at species level using the Blast

AMB1

in

the

comix

culture,

the

and

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AMB1_1028F

AMB1_1227R

(5´(5´-

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algorithm31 provided by the National Center for Biotechnology Information (NCBI

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http://www.ncbi.nlm.nih.gov). Raw sequences were submitted to the NCBI Sequence Read

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Archive (SRA) under the study accession number PRJNA514445.

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Cultivation Experiments. Two different cultivation experiments were conducted in this study,

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focusing on I) analysis of thermodynamics and II) determination of growth parameters for

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optimized methane production rates and calculation of doubling times.

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Experiment I) Cultivation and thermodynamic calculations. Triplicate anaerobic batches

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of each culture (cos and comix) were prepared using 200 mM acetate, 0.2 M NH4Cl, and initial

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pH (pHinitial) of 7.3. Incubation was at 37°C, giving a free ammonia level of 0.09 g NH3-N/L.

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The cultures were grown in 0.5 L serum bottles, containing 0.25 L media and were inoculated

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with 12.5 mL of co-culture that had depleted acetate to below detection. Triplicate cultures

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incubated in medium without acetate served as negative controls. Determination of gas

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composition (H2, CH4, and CO2) and analyses of liquid samples (pH, acetate and 16S rRNA

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gene abundance) were conducted throughout. Liquid samples of 1 mL for DNA extraction were

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collected during growth and stored at -20°C until further analysis. For the thermodynamic

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calculations, the reactions evaluated were: CH3COO- + H+ + 2H2O → 2CO2 + 4H2 (reaction 1;

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ΔG° = 55.0 kJ), 4H2 + CO2 → CH4 + 2H2O (reaction 2; ΔG° = -130.8 kJ), and CH3COO- + H+

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→ CH4 + CO2 (reaction 3; ΔG° = -75.8 kJ). Temperature corrections for 37°C versus 25°C (the

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standard temperature) were made using the Gibbs-Helmholz equation, with H2, CO2, and CH4

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in the gas phase (standard conditions: partial pressure at 1 atm), and acetate in the aqueous

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phase (standard concentration at 1 M).32 Gf and Hf values were taken from Hanselmann.33 Gibbs

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free energy (ΔG) values pertaining to actual concentrations and partial pressures were

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calculated using the Nernst equation, as described previously.32 All calculation procedures are

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described in detail in Dolfing.34

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Kinetic parameters. The generation time was calculated from the qPCR results using the

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logarithmic growth equation Nt = N0 × eµt, where Nt is the number of cells at time t, N0 is the

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number of cells at time zero, and µ is the growth rate constant. The value of µ (assumed

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constant) was calculated from the slope of the 16S rRNA gene increase during the period of

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exponential growth. The generation time (g) was calculated as g = (ln2)/µ, an expression

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derived from the logarithmic growth equation. The acetate threshold level was determined in

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these cultures after 100-200 days of cultivation.

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Experiment II) Determination of methane production rates at different pH, temperature,

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ammonia and acetate levels and calculation of doubling times. The comix culture experiment

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was intended to generate data relevant for efforts to improve operating strategies in biogas

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digesters, particularly regarding the impact on methane production rate of temperature,

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ammonium level, and initial acetate concentration. The experiment was set up using the design-

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of-experiment approach (Modde software v. 11, Umetrics AB, Umeå, Sweden) and was run in

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two sets, at pHinitial 7.3 and at pHinitial 8.1. The range of the factors for both pH levels was set at

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0.05-0.34 M NH4Cl, 30-46°C, and 0.05-0.4 M sodium acetate (Table S1.1), with the intention

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of mimicking typical biogas digester conditions. The cultures were grown in 0.25 L serum

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bottles, containing 0.08 L media and were inoculated with 4 mL of co-culture that had depleted

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acetate to below detection. Methane yield was monitored one to two times a week until gas

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production ceased, and the logarithmic increase in methane concentration in the individual

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batches was recorded as the response factor. Response surface methodology (RSM), which

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evaluates the data with multiple linear regression, and a central composite face-centered design

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with three levels (low, middle, and high) were used in the Modde software to conduct the full

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factorial design. Duplicate samples at each set point were analyzed and three replicates of the

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central point were included in the design, to give a final experimental matrix of 60 batch

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experiments, in total representing 15 different set-up conditions, at each pH level (Table S1.1).

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Methane production and acetate degradation were measured throughout. The doubling times

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(td,CH4) were estimated using the specific methane production rate (CH4) in the equation td,CH4

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= ln2/CH4, where CH4 was calculated from the slope of logarithmic methane increase during

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exponential methane production.

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RESULTS AND DISCUSSION

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To better understand the kinetics and ecophysiology of the organisms involved in syntrophic

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acetate oxidation, we created two syntrophic acetate-oxidizing communities, cos and comix.

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Both communities relied on M. bourgensis as the hydrogen scavenger. This methanogen is an

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efficient hydrogen consumer in mesophilic SAO cultures8-10 and is prevalent in SAO-

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dominated biogas systems.35, 36 The syntrophic acetate oxidizer in cos was S. schinkii, while the

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syntrophic comix community consisted of S. schinkii, [C.] ultunense and T. acetatoxydans.

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However, 16S rRNA gene Illumina sequencing revealed presence of an uncharacterized

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species, strain AMB1 in the M. bourgensis culture and it was thus also included in the cos and

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comix cultures.

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Acetate consumption and methane production were equimolar in SAO cultures. Analysis

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of acetate and methane concentrations in the cos and comix cultures during growth revealed a

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1:1 ratio between consumption of acetate and production of methane (Figures 1a and 2a), which

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is in agreement with previous findings for mesophilic and thermophilic SAO cultures.11, 20 This

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demonstrates the metabolic interdependence and tight coupling between the bacteria and the

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methanogen.

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Hydrogen partial pressures and Gibbs free energy changes stabilize in SAO cultures.

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Production and consumption of four moles of hydrogen per mole of acetate oxidized, and per

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mole of methane produced, means that the amount of energy available from both reactions is

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very sensitive to the hydrogen partial pressure. Thus pH2 can be expected to stay within a

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narrow range, as both reactions need to be exergonic if the organisms involved are to obtain

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energy for growth from these reactions. We found this expectation to be fulfilled in both

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cultures. Except for early pH2 peaks of 10 Pa in cos after 15 days and 7 Pa after 8 days in comix,

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pH2 essentially remained consistently between 3.1 and 5.3 Pa (average 4.2 Pa) over the course

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of the growth experiments in both cos and comix (Fig 1a and 1b). pH increased from 7.3 to 7.9-

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8.0 and CO2 varied between 12-29% in all cultures during growth (Table S1.2).

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Thermodynamic calculations demonstrated that both acetate oxidation and hydrogenotrophic

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methanogenesis were exergonic at all times and that the energetics in cos and comix were

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consistent. In both cultures, the ΔG values started out at levels of about -30 to -40 kJ/reaction

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for acetate oxidation and hydrogenotrophic methanogenesis, respectively, and stabilized at -10

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kJ/mol for acetate oxidation and -20 kJ/mol for hydrogenotrophic methanogenesis (Figures 3

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and S1.1). Thus the methanogens obtained more energy from this partnership than their acetate-

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oxidizing partners. This is different to a previously analyzed methanogenic SAO tri-culture

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including M. bourgensis and [C.] ultunense, in which equal sharing was assumed (i.e. 17 kJ/mol

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each).20 The hydrogen levels in that study [1.6-6.8 Pa] were similar to the steady state levels

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observed here, and substantially lower than those typically observed in thermophilic SAO-

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cultures (10-60 Pa).19,

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opportunity and allows for higher hydrogen levels.32

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Idiosyncratic growth of the SAO bacteria and the methanogen. Given that the hydrogen

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partial pressure stayed within a narrow range during our experiments, one would expect

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methane production to result in growth of the methanogen throughout. We found that this was

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not the case. In both communities, 16S rRNA gene copies of the methanogen ceased halfway

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through the experiment (Figures 1b and 2b). Nevertheless, after growth had ceased methane

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production continued at a steady pace, demonstrating that the methanogenic population was

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still highly active. During the period of exponential growth, i.e., about day 70 to 100 in cos and

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This was expected, since temperature increases the window of

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day 8 to 30 in comix, the methanogen increased from 106-7 to 108 gene copies/mL, giving

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generation times of 20 days in cos and 9 days in comix (Table 1).

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Growth of the SAO bacteria was even more idiosyncratic. In cos, the 16S rRNA gene copy

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numbers of S. schinkii increased steadily between days 50 and 80 to reach 108 gene copies/mL

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(Figure 1b). After this, growth of S. schinkii continued, but at a lower rate, until day 100, when

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growth of S. schinkii stopped and copy numbers tended to decrease, even though there was still

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plenty of acetate (100 mM) present, and acetate continued to be degraded until it was fully

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depleted at day 160 (Figure 1a). A similar pattern was seen for comix, where exponential growth

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of S. schinkii at its initial ‘maximum’ rate ceased at 108 gene copies/mL (~ day 30) (Figure 2b,

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Table SI.3), a point where there was still a lot of acetate present. Just as in cos, growth of S.

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schinkii continued after this, but at a lower rate (Figures 2b). [C.] ultunense and strain AMB1

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grew faster than S. schinkii, but growth of these organisms stopped earlier than for S. schinkii.

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Thus S. schinkii also became the dominant microorganism in comix (Figures 2b and 4). Another

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interesting observation is that S. schinkii reached similar abundance in both cos and comix, and

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thus the fact that it had to share the available substrate with other syntrophic acetate-oxidizing

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bacteria appeared not to affect its growth. Analyses of cultures without acetate suggested that

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[C.] ultunense, and in particular strain AMB1, grew on yeast extract (Table SI.3). This implies

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that, even in cultures with acetate, the initial rapid increase in [C.] ultunense and strain AMB1

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during the first week of incubation was due to growth on yeast extract. Detection of traces of

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propionate and butyrate in comix at the end of the experiment supports this hypothesis. However,

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after the initial rapid increase, [C.] ultunense and AMB1 continued to increase, but at a slower

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pace. At days 30-40, [C.] ultunense abundance reached higher levels in cultures with acetate

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(1-2 × 108 gene copies/mL) than in cultures without acetate (4 × 107 gene copies/mL),

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illustrating its ability to oxidize acetate. For AMB1, there was no difference between cultures

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with and without acetate (108 gene copies/mL in all cultures), so the ability of this bacterial

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species to oxidize acetate remains to be investigated. Still, the fact that strain AMB1 did not

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show any growth in the cos culture suggests that its growth on yeast and/or acetate was

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regulated by the presence of [C.] ultunense or T. acetatoxydans. The slow growth and low gene

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abundance of T. acetatoxydans (Figure 2b), particularly considering that this species has two

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16S rRNA copy numbers per genome whereas M. bourgensis sp. MAB1, S. schinkii and [C.]

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ultunense have one38-40, indicate a restricted metabolic contribution of T. acetatoxydans in the

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comix culture.

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The Illumina sequencing supported the qPCR results and showed dominance of S. schinkii in

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both cultures (Figure 4). In addition, strain AMB1 was only detected in the Illumina sequencing

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in samples taken at the first days in the cos culture and likely did not to grow, as it was not

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detected after 50 days of incubation. This was further strengthened using the AMB-targeting

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primers in qPCR analysis, which indicated no presence of this species above the detection limit

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of 100 gene copies/mL in any of the samples. Moreover, in the Illumina analysis, sequences

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classified into the bacterial genus Chungangia were detected in cos at days 5-48. Chungangia

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is strict aerobic bacteria41 that is unlikely to grow in these anaerobic cultures. These sequences

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were thus considered to represent DNA contamination of extraction and sequencing reagents

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appearing in the analysis, due to the extremely low microbial biomass in the initial days of

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cultivation. Similarly to the qPCR results, the Illumina analysis also showed higher relative

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abundance of SAO bacteria than of the methanogen, even considering differences in 16S rRNA

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copy numbers per genome (Figure 4). This was rather unexpected, as the energy available from

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acetate oxidation was lower than that from methanogenesis. The reason for this is not

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immediately clear from the present results, but it can be speculated that the methanogen may

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have to invest more energy in assimilation (e.g. the synthesis of amino acids), whereas the SAO

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microorganisms may take more advantage of the yeast extract in the medium or use secondary

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metabolites from the methanogen. Another possibility could be that the methanogen simply

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dissipates more of the free energy and has a lower energy gain than the SAO microorganisms.

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One interesting dissimilarity between the comix and cos cultures was the number of days

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required for initiation of methane production after inoculation (8 days for comix, 83 days for

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cos). This may be taken to suggest that one or more of the other organisms in the comix

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community (viz. T. acetatoxydans or [C.] ultunense) provided a factor that somehow lowered

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the threshold for initiation of SAO. It also appeared to expedite growth of S. schinkii and M.

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bourgensis, which grew faster in comix than in cos (Table 1). These differences between comix

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and cos are not only intriguing, but also relevant, because they show that the more complex

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comix community instigated more efficient acetate degradation than the simpler cos community.

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This indicates that information gleaned from studying a simple community cannot be directly

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extrapolated to the ‘real world’. Mesophilic anaerobic digesters in which the SAO route

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dominates are complex and show more resemblance to the comix community than to the cos

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community. There are generally a number of syntrophic acetate oxidizers present in SAO-

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dominated biogas systems, but S. schinkii is often the most abundant of the known syntrophic

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bacteria23, 35, 42. This was also the case in the comix culture. Overall, our results indicate that

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cooperation between a consortium benefits the growth of syntrophic acetate oxidizers,

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confirming suggestions in previous research that syntrophy in the ‘real world’ is more complex

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than previously thought.43

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Effects of environmental conditions on the methane production rate. Growth experiments

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and modeling of synthetic communities are useful to generate predictions of how different

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parameters control methane production in more complex systems. The main aim of the present

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experiment was to gain insights into the ecophysiology of syntrophic acetate oxidizers under

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prevalent biogas process conditions and the experimental set-up was therefore designed to

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replicate this environment. The parameters tested were temperature, pH, ammonia and acetate

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levels. The experiment was performed on comix due to its higher resemblance to the diverse

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SAO consortia prevailing in biogas systems.5 The model obtained from methane production

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rates at varying growth conditions was shown to describe the variation in the data with high

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accuracy (Table SI.4). Under the conditions examined, temperature proved to have a strong

321

impact on methane formation, with the highest production rates obtained at around 42-46C at

322

both pHinitial 7.3 and 8.1 (Figure 5, 6 and SI.2). This temperature range resembles the

323

heterotrophic growth pattern of T. acetatoxydans,10 whereas [C.] ultunense had its highest

324

growth rate around 37°C.8 The effect of temperature on the growth rate of S. schinkii and strain

325

AMB1 has not been determined in pure culture. However, the upper temperature limit of C.

326

ultunense strain Esp and S. schinkii during heterotrophic growth (40-45°C)9 and the presence

327

of relatively low numbers of heat shock proteins in their genomes17, 44 raise many questions

328

regarding the interplay of the different species in comix at higher temperatures. Whether [C.]

329

ultunense and S. schinkii benefit from SAO conditions and/or other strains in the co-culture

330

and remain active at 42-46°C, and whether T. acetatoxydans and/or strain AMB1 is the main

331

acetate consumer(s) in this setting, remain to be established. For practical application, this comix

332

optimum range lies in between the mesophilic (35-38°C) and thermophilic (50-60°C)

333

temperature intervals commonly applied in commercial biogas production.45 Previous studies

334

performed in our laboratory have assessed this temperature interval for its suitability for biogas

335

production under high ammonia conditions, with the aim of supporting SAO activity.35, 46 One

336

such study revealed positive effects on methane production, enhanced degradation of amino

337

acids, and increased abundance of T. acetatoxydans in degradation of thin stillage at 44°C

338

instead of 38°C.46 However, in processes fed household waste supplemented with protein, a

339

similar temperature increase (from 37°C to 42°C) had less effect on methane yield and on the

340

abundance of known SAO bacteria.35

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An important aspect when considering the impact of temperature is its effect on ammonia level.

342

Increased temperature shifts the equilibrium between ammonium (NH4+) and ammonia (NH3)

343

towards the latter, which is mainly responsible for inhibition of the microbial community.47 In

344

our experiments, the higher temperature resulted in ammonia levels of 0.4 and 1.8 g NH3/L at

345

pHinitial 7.3 and 8.1, respectively. The continued methane formation at the higher ammonia level

346

demonstrates extremely high ammonia tolerance of the syntrophs involved, which confirms

347

previous findings for pure cultures of syntrophic bacteria.8-10,

348

ammonium uptake systems and encoding of potassium uptake proteins may be potential

349

underlying mechanisms.15, 17, 40, 44, 48 Our cultivation experiments even showed a positive effect

350

of higher ammonia levels on methane production rate, which is likely to be an highly important

351

selective factor for establishing SAO in high-ammonia biogas systems.

352

The thermodynamic benefit of high acetate concentrations6 was reflected in enhanced rates of

353

methane production by comix at higher acetate levels. Maximum methane production rates were

354

obtained at around 0.2-0.3 M (Figures 5, 6 and SI.2). Interestingly, the upper level of acetate

355

seems to be slightly inhibitory at 7.3 but not at 8.1 (Figures 5 and 6), which might indicate a

356

pH dependent inhibitory effect by the undissociated form of acetate on the methane production

357

rate. Genome-based analyses will be helpful in obtaining further information about the impact

358

of acetate on the SAO community, but the indication that T. acetatoxydans possesses a passive

359

rather than active acetate uptake system15 could be an explanation for higher growth of the

360

comix culture at the higher acetate levels. Note that the optimum acetate concentration (0.2-0.40

361

M, 12-24 g/L) predicted in the present study for the comix culture is an extremely high level for

362

commercial biogas production, but can still be found in ammonia-inhibited systems.4, 49

363

Competition with aceticlastic methanogens at high and low acetate levels in biogas

364

processes. The results obtained here were used to estimate kinetic parameters describing the

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The absence of genes for

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growth of SAO organisms and to provide a basis for comparison of our data with previous

366

studies of aceticlastic methanogens. Using qPCR results for the period of exponential growth,

367

generation times between 3-12 days were estimated for all the syntrophic microorganisms

368

involved except strain AMB1 (Table 1). This exceeds the generation time reported for

369

Methanosarcina sp. (0.5-2 days), but is in a similar range as Methanosaeta (3.5-12 days sp.).50

370

The higher growth rate of Methanosarcina and the high acetate affinity of Methanosaeta

371

(further discussed below) indicate that SAOs have low competitiveness against aceticlastic

372

methanogens in non-stressed environments. However, the generation times of these aceticlastic

373

methanogens were obtained when grown at one set of parameters (35°C, low ammonia, pH 7.2

374

etc.) and parameters such as acetate, pH, ammonia level and temperature will most likely effect

375

their competitiveness. It is well known that the lower ammonia tolerance of aceticlastic

376

methanogens often causes SAO dominance in high-ammonia environments.5 Still, the most

377

rapid doubling times obtained in the present study (Table S1.5) also indicate SAO

378

competiveness relative to aceticlastic methanogens in systems operating with low and moderate

379

ammonia levels, if other conditions favor SAO. This would explain the SAO dominance

380

reported at high temperature and/or high acetate in the absence of high ammonia as a selective

381

factor.51-55

382

The minimum threshold for acetate utilization was 0.40-0.45 mM in the cos culture and 0.7

383

mM in the comix culture (Table SI.6), which is comparable to the acetate affinity of

384

Methanosarcina (0.2-2.5 mM).56, 57 However, the minimum acetate level for Methanosarcina

385

was determined in low-ammonia conditions and may be different when it is grown under higher

386

ammonia levels, as used in the present study. Our data therefore indicate that SAO

387

microorganisms can compete for acetate even when acetate is present at low levels, as

388

confirmed by the dominance of SAO reported in biogas digesters operating at low acetate levels

389

and high ammonia concentrations.5,

58

The result of the present study also shows that the

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minimum threshold for acetate utilization of SAO microorganisms considerably exceeds the

391

level of 7-70 µM reported for Methanoseata which is the other methanogenic group competing

392

for acetate.59 Consequently, SAO microorganisms will not be able to compete with

393

Methanosaeta, in absence of inhibitory compounds and when acetate is the limiting parameter.

394

However, Methanosaeta sp. have low tolerance to specific inhibitors and are seldom detected

395

in high-ammonia biogas processes.5

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SUPPORTING INFORMATION

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The supporting information accompanying this manuscript contains information relating to:

398



methods involving of factors of the experimental design used in experiment II

399



results of performance of the experimental design, average 16S rRNA gene copy

400

numbers of all strains when incubated with and without acetate, estimated doubling

401

time (during growth at different temperatures, acetate concentrations, ammonia levels,

402

and pHinitial), detailed values of minimum threshold for acetate utilization, change in

403

Gibbs free energy over time and impact of acetate concentration and temperature on

404

methane production rates (at different ammonia levels) by the comix culture at pHinitial

405

7.3.

406

ACKNOWLEDGEMENTS

407

We thank Anna Neubeck, Abhijeet Singh and Simon Isaksson for assistance in sampling and

408

analyses of gas composition. MW and AS thanks the Swedish University of Agricultural

409

Sciences for financial support. JD acknowledges funding from the Biotechnology and

410

Biological Sciences Research Council (BB/K003240/1; Engineering synthetic microbial

411

communities for biomethane production).

412

REFERENCES

413 414 415 416 417 418 419 420 421 422 423

(1) (2) (3) (4)

Lauer, M.; Hansen, J. K.; Lamers, P.; Thran, D., Making money from waste: The economic viability of producing biogas and biomethane in the Idaho dairy industry Appl. Energ. 2018, 222, 621-636. Moestedt, J.; Nilsson Påledal, S.; Schnürer, A.; Nordell, E., Biogas production from thin stillage on an industrial scale - experience and optimisation. Energies 2013, 6, 5642-5655. Chen, J. L.; Ortiz, R.; Steele, T. W. J., Toxicants inhibiting anaerobic digestion: A review. Biotechnol. Adv. 2014, 32, 1523-1534. Schnürer, A.; Nordberg, A., Ammonia, a selective agent for methane production by syntrophic acetate oxidation at mesophilic temperature. Water Sci. Technol. 2008, 57, 735-740.

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Page 19 of 29

424 425 426 427 428 429 430 431 432 433 434 435 436 437 438 439 440 441 442 443 444 445 446 447 448 449 450 451 452 453 454 455 456 457 458 459 460 461 462 463 464 465 466 467 468 469 470 471 472

Environmental Science & Technology

(5) (6) (7) (8)

(9) (10)

(11) (12) (13)

(14) (15)

(16) (17)

(18)

(19)

Westerholm, M.; Moestedt, J.; Schnürer, A., Biogas production through syntrophic acetate oxidation and deliberate operating strategies for improved digester performance. Appl. Energ. 2016, 179, 124-135. Dolfing, J., Thermodynamic constraints on syntrophic acetate oxidation. Appl. Environ. Microbiol. 2014, 80, 1539-1541. Stams, A. J. M., Metabolic interactions between anaerobic bacteria in methanogenic enviroments. Antonie van Leeuwenhoek 1994, 66, 271-294. Schnürer, A.; Schink, B.; Svensson, B. H., Clostridium ultunense sp. nov., a mesophilic bacterium oxidizing acetate in syntrophic association with a hydrogenotrophic methanogenic bacterium. Int. J. Syst. Bacteriol. 1996, 46, 11451152. Westerholm, M.; Roos, S.; Schnürer, A., Syntrophaceticus schinkii gen. nov., sp. nov., an anaerobic, syntrophic acetate-oxidizing bacterium isolated from a mesophilic anaerobic filter. FEMS Microbiol. Lett. 2010, 309, 100-104. Westerholm, M.; Roos, S.; Schnürer, A., Tepidanaerobacter acetatoxydans sp. nov., an anaerobic, syntrophic acetate-oxidizing bacterium isolated from two ammoniumenriched mesophilic methanogenic processes. Syst. Appl. Microbiol. 2011, 34, 260266. Hattori, S.; Kamagata, Y.; Hanada, S.; Shoun, H., Thermacetogenium phaeum gen. nov., sp. nov., a strictly anaerobic, thermophilic, syntrophic acetate-oxidizing bacterium. Int. J. Syst. Evol. Microbiol. 2000, 50, 1601-1609. Balk, M.; Weijma, J.; Stams, A. J. M., Thermotoga lettingae sp. nov., a novel thermophilic, methanol-degrading bacterium isolated from a themophilic anaerobic reactor. Int. J. Syst. Evol. Microbiol. 2002, 52, 1361-1368. Bhandari, V.; Gupta, R. S., Molecular signatures for the phylum (class) Thermotogae and a proposal for its division into three orders (Thermotogales, Kosmotogales ord. nov. and Petrotogales ord. nov.) containing four families (Thermotogaceae, Fervidobacteriaceae fam. nov., Kosmotogaceae fam. nov. and Petrotogaceae fam. nov.) and a new genus Pseudothermotoga gen. nov. with five new combinations. Antonie van Leeuwenhoek 2014, 105, 143-168. Hattori, S., Syntrophic acetate-oxidizing microbes in methanogenic environments. Microbes Environ. 2008, 23, 118-127. Müller, B.; Manzoor, S.; Niazi, A.; Bongcam-Rudloff, E.; Schnürer, A., Genomeguided analysis of physiological capacities of Tepidanaerobacter acetatoxydans provides insights into environmental adaptations and syntrophic acetate oxidation. PLoS ONE 2015, 10, 1-21. Müller, B.; Sun, L.; Schnürer, A., First insights into the syntrophic acetate-oxidizing bacteria - a genetic study. MicrobiologyOpen 2012, 2, 35-53. Manzoor, S.; Schnürer, A.; Bongcam-Rudloff, E.; Müller, B., Genome-guided analysis of Clostridium ultunense and comparative genomics reveal different strategies for acetate oxidation and energy onservation in syntrophic acetateoxidising bacteria. Genes 2018, 9, 225. Oehler, D.; Poehlein, A.; Leimbach, A.; Müller, N.; Daniel, R.; Gottschalk, G.; Schink, B., Genome-guided analysis of physiological and morphological traits of the fermentative acetate oxidizer Thermacetogenium phaeum. BMC Genomics 2012, 13, 723. Hattori, S.; Luo, H.; Shoun, H.; Kamagata, Y., Involvement of formate as an interspecies electron carrier in a syntrophic acetate-oxidizing anaerobic microorganism in coculture with methanoges. J. Biosci. Bioeng. 2001, 91, 294-298.

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Environmental Science & Technology

473 474 475 476 477 478 479 480 481 482 483 484 485 486 487 488 489 490 491 492 493 494 495 496 497 498 499 500 501 502 503 504 505 506 507 508 509 510 511 512 513 514 515 516 517 518 519 520 521

(20) (21) (22) (23) (24) (25) (26) (27) (28) (29) (30) (31) (32) (33) (34)

(35) (36) (37) (38)

Schnürer, A.; Svensson, B. H.; Schink, B., Enzyme activities in and energetics of acetate metabolism by the mesophilic syntrophically acetate-oxidizing anaerobe Clostridium ultunense. FEMS Microbiol. Lett. 1997, 154, 331-336. Schnürer, A.; Zellner, G.; Svensson, B. H., Mesophilic syntrophic acetate oxidation during methane formation in biogas reactors. FEMS Microbiol. Ecol. 1999, 29, 249261. Jonsson, S.; Boren, H., Analysis of mono- and diesters of o-phthalic acid by solidphase extractions with polystyrene-divinylbenzene-based polymers. J. Chromatogr. 2002, 963, 393-400. Westerholm, M.; Dolfing, J.; Sherry, A.; Gray, N. D.; Head, I. M.; Schnürer, A., Quantification of syntrophic acetate-oxidizing microbial communities in biogas processes. Environ. Microbiol. Report. 2011, 3, 500-505. Westerholm, M.; Hansson, M.; Schnürer, A., Improved biogas production from whole stillage by co-digestion with cattle manure Bioresour. Technol. 2012, 114, 314-319. Westerholm, M.; Isaksson, S.; Karlsson Lindsjö, O.; Schnürer, A., Microbial community adaptability to altered temperature conditions determines the potential for process optimisation in biogas production. Appl. Energ. 2018, 226, 838-848. Chen, S.; Zhou, Y.; Chen, Y.; Gu, J., fastp: an ultra-fast all-in-one FASTQ preprocessor. Bioinformatics 2018, 34, (17), 884-890. Callahan, B. J.; McMurdie, P. J.; Rosen, M. J.; Han, A. W.; Johnson, J. A.; Holmes, S. P., DADA2: High-resolution sample inference from Illumina amplicon data. Nat. Methods 2016, 13, 581-583. McMurdie, P. J.; Holmes, S., phyloseq: An R package for reproducible interactive analysis and graphics of microbiome census data. PLoS ONE. 2013, 8, e61217. Wickham, H., ggplot2: Elegant graphics for data analysis. In Springer-Verlag: New York, NY, USA, 2016. Team, R. RStudio: Integrated Development for R. RStudio, Inc., Boston, MA URL Website; http://www.rstudio.com/, 2016. Altschul, S. F.; Gish, W.; Miller, W.; Myers, E. W.; Lipman, D. J., Basic local alignment search tool. J. Mol. Biol. 1990, 215, 403-410. Dolfing, J.; Larter, S. R.; Head, I. M., Thermodynamic constraints on methanogenic crude oil biodegradation. ISME J. 2008, 2, 442-452. Hanselmann, K. W., Microbial energetics applied to waste repositories. Experientia 1991, 47, 645-687. Dolfing, J., Protocols for calculating reaction kinetics and thermodynamics. In Hydrocarbon and Lipid Microbiology Protocols, Springer Protocols Handbooks; McGenity T., Timmis K., Nogales Fernández B., Eds.; Springer-Verlag: Berlin, 2015; pp 155-163. Westerholm, M.; Müller, B.; Isaksson, S.; Schnürer, A., Trace element and temperature effects on microbial communities and links to biogas digester performance at high ammonia levels. Biotechnol. Biofuel. 2015, 8, 1-19. Westerholm, M.; Müller, B.; Singh, A.; Karlsson Lindsjö, O.; Schnürer, A., Detection of novel syntrophic acetate-oxidising bacteria from biogas processes by continuous acetate enrichment approaches. Microbial Biotechnol. 2018, 11, 680-693. Lee, M. J.; Zinder, S. H., Hydrogen partial pressure in a thermophilic acetateoxidizing methanogenic coculture. Appl. Environ. Microbiol. 1988, 54, 1457-1461. Manzoor, S.; Bongcam-Rudloff, E.; Schnürer, A.; Müller, B., First genome sequence of a syntrophic acetate-oxidizing bacterium, Tepidanaerobacter acetatoxydans strain Re1 Genome Announc. 2013, 1, e00213-12.

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Environmental Science & Technology

(39) (40) (41) (42) (43) (44) (45) (46) (47) (48)

(49) (50) (51) (52) (53) (54) (55)

Manzoor, S.; Müller, B.; Niazi, A.; Bongcam-Rudloff, E.; Schnürer, A., Draft genome sequence of Clostridium ultunense strain Esp, a syntrophic acetate-oxidizing bacterium. Genome Announc. 2013, 1, e00107-13. Manzoor, S.; Schnürer, A.; Bongcam-Rudloff, E.; Müller, B., Complete genome sequence of Methanoculleus bourgensis strain MAB1, the syntrophic partner of mesophilic acetate-oxidising bacteria (SAOB). Stand. Genom. Sci. 2016, 1-9. Kim, W.; Traiwan, J.; Park, M. H.; Jung, M. Y.; Oh, S. J.; Yoon, J. H.; Sukhoom, A., Chungangia koreensis gen. nov., sp nov., isolated from marine sediment Int. J. Syst. Evol. Microbiol. 2012, 62, 1914-1920. Westerholm, M.; Levén, L.; Schnürer, A., Bioaugmentation of syntrophic acetateoxidising culture in biogas reactors exposed to increasing levels of ammonia. Appl. Environ. Microbiol. 2012, 78, 7619-7625. Nobu, M. K.; Narihiro, T.; Rinke, C.; Kamagata, Y.; Tringe, S. G.; Woyke, T.; Liu, W., Microbial dark matter ecogenomics reveals complex synergistic networks in a methanogenic bioreactor. ISME J. 2015, 9, 1710-1722. Manzoor, S.; Bongcam-Rudloff, E.; Schnürer, A.; Müller, B., Genome-guided analysis and whole transcriptome profiling of the mesophilic syntrophic acetate oxidising bacterium Syntrophaceticus schinkii PLoS ONE 2015, 11, e0166520. Kim, M.; Ahn, Y. H.; Speece, R. E., Comparative process stability and efficiency of anaerobic digestion; mesophilic vs. thermophilic. Water Res. 2002, 36, 4369-4385. Moestedt, J.; Nordell, E.; Schnürer, A., Comparison of operational strategies for increased biogas production from thin stillage. J. Biotechnol. 2014, 175, 22-30. Sprott, G. D.; Shaw, K. M.; Jarell, K. F., Ammonia/potassium exchange in methanogenic bacteria. J. Biol. Chem. 1984, 259, 12602-12608. Maus, I.; Wibberg, D.; Stantscheff, R.; Stolze, Y.; Blom, J.; Eikmeyer, F.; Fracowiak, J.; König, H.; Pühler, A.; Schlüter, A., Insights into the annotated genome sequence of Methanoculleus bourgensis MS2T, related to dominant methanogens in biogasproducing plants. J. Biotechnol. 2015, 201, 43-53. Moestedt, J.; Müller, B.; Westerholm, M.; Schnürer, A., Ammonia threshold for inhibition of anaerobic digestion of thin stillage and the importance of organic loading rate. Microbial Biotechnol. 2016, 9, (2), 180-194. Yu, Y.; Kim, J.; Hwang, S., Use of real-time PCR for group-specific quantification of aceticlastic methanogens in anaerobic processes: population dynamics and community structure. Biotechnol. Bioeng. 2005, 93, 424-433. Ho, D.; Jensen, P.; Gutierrez-Zamora, M.; Beckmann, S.; Manefield, M.; Batstone, D., High-rate, high temperature acetotrophic methanogenesis governed by a three population consortium in anaerobic bioreactors. PLoS ONE 2016, 11, e0159760. Ho, D.; Jensen, P.; Batstone, D., Effects of temperature and hydraulic retention time on acetotrophic pathways and performance in high-rate sludge digestion. Environ. Sci. Technol. 2014, 48, 6468-6476. Hao, L.; Lü, F.; Wu, Q.; Shao, L.; He, P., Self-adaptation of methane-producing communities to pH disturbance at different acetate concentrations by shifting pathways and population interaction. Bioresour. Technol. 2013, 140, 319-327. Petersen, S. P.; Ahring, B. K., Acetate oxidation in a thermophilic anaerobic sludgedigestor: the importance of non-acetoclastic methanogenesis from acetate. FEMS Microbiol. Ecol. 1991, 86, 149-158. Hao, L.; Lü, F.; He, P.; Li, L.; Shao, L., Predominant contribution of syntrophic acetate oxidation to thermophilic methane formation at high acetate concentrations. Environ. Sci. Technol. 2011, 45, 508-513.

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(56) (57) (58) (59)

Jetten, M. S. M.; Stams, A. J. M.; Zehnder, A. J. B., Acetate threshold values and acetate activating enzymes in methanogenic bacteria. FEMS Microbiol. Ecol. 1990, 73, 339-344. Zinder, S. H., Conversion of acetic acid to methane by thermophiles. FEMS Microbiol. Rev. 1990, 75, 125-138. Ahring, B. K., Methanogenesis in thermophilic biogas reactors. Antonie van Leeuwenhoek 1995, 67, 91-102. Jetten, M. S. M.; Stams, A. J. M.; Zehnder, A. J. B., Methanogenesis from acetate: a comparison of the acetate metabolism in Methanothrix soehngenii and Methanosarcina spp. FEMS Microbiol. Rev. 1992, 88, 181-198.

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Table 1. Generation time estimated from the qPCR results for triplicate cultures of cos and

583

comix when incubated at 37°C in medium containing 200 mM acetate, 0.2 M NH4Cl, and an

584

initial pH of 7.3. The equation g = (ln2)/µ was used for calculation, where µ (assumed constant)

585

was estimated from the slope of the logarithmic increase in 16S rRNA genes of the respective

586

species

culture

Syntrophaceticus schinkii

[Clostridiu m] ultunense

Tepidanaerobacte r acetatoxydans

strain AMB1

Methanoculleus bourgensis

cos

19.7 ± 1.51

np

np

np

19.8 ± 1.42

comix

9.5 ± 0.53

4.5 ± 0.24

11.7 ± 0.54

3.1 ± 0.14

8.5 ± 0.43

587

np = not present

588

1 Time

589

for calculation: days 8-28; 4 Time frame used for calculation: days 0-14 (the qPCR data used for the calculations

590

are shown in Figures 1b and 2b)

frame used for calculation: days 48-83; 2 Time frame used for calculation: days 74-96; 3 Time frame used

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591

a

b

592 593

Figure 1. (a) Acetate consumption, methane formation, and hydrogen partial pressure and (b)

594

the 16S rRNA gene abundances (determined through qPCR analyses) of Syntrophaceticus

595

schinkii and Methanoculleus bourgensis during 200 days of co-cultivation of the cos culture.

596

qPCR analyses using primers designed to target strain AMB1 showed no detection of this

597

species in cos. The co-cultures contained 0.2 M NH4Cl and an initial acetate concentration of

598

200 mM (equal to 40 mmol per bottle), and were incubated at 37°C. Each sample point

599

represents an average of triplicate biological replicates.

600

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a

b

602

603 604

Figure 2. (a) Acetate consumption, methane formation, and hydrogen partial pressure and (b)

605

16S rRNA gene copies (determined through qPCR analyses) of Syntrophaceticus schinkii,

606

[Clostridium] ultunense, Tepidanaerobacter acetatoxydans, strain AMB1, and Methanoculleus

607

bourgensis during 120 days of co-cultivation of the comix culture. The co-cultures contained

608

0.2 M NH4Cl and an initial acetate concentration of 200 mM (equal to 40 mmol per bottle),

609

and were incubated at 37°C. Each sample point represents an average of triplicate biological

610

replicates.

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611 612

Figure 3. Change in Gibbs free energy (ΔG) for acetate oxidation (left panel) and

613

hydrogenotrophic methanogenesis (right panel) in the cos culture (green symbols) and in the

614

comix culture (red symbols) during acetate degradation.

615

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Figure 4. Relative abundance at genus level (based on total sequences) in the comix culture

618

(Syntrophaceticus schinkii, [Clostridium] ultunense, Tepidanaerobacter acetatoxydans, strain

619

AMB1, and Methanoculleus bourgensis) and the cos culture (S. schinkii, strain AMB1, and M.

620

bourgensis) during degradation of 40 mmol (equal to 200 mM per bottle) acetate as shown in

621

Figures 2a and 3a. The results are mean values of biological triplicate batches. Blast searches

622

of the representative sequences revealed that Tepidimicrobium-classified reads had 97-99%

623

sequence similarity to [C.] ultunense and that the majority of the unclassified reads (NA in the

624

diagram) had 100% sequence similarity to the novel strain AMB1.

625

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Figure 5. Impact of acetate concentration and temperature on methane production rates by the

629

comix culture (Syntrophaceticus schinkii, [Clostridium] ultunense, Tepidanaerobacter

630

acetatoxydans, strain AMB1, and Methanoculleus bourgensis) at 0.05, 0.225, and 0.4 M acetate

631

concentrations and pHinitial 7.3. The parameters investigated were within the ranges 0.05-0.34

632

M NH4Cl, 30-46°C, and 0.05-0.4 M sodium acetate.

633 634

635 636

Figure 6. Co-cultivation at pHinitial 8.1 and the impact of acetate and ammonia on methane

637

production rates by the comix culture (Syntrophaceticus schinkii, [Clostridium] ultunense,

638

Tepidanaerobacter acetatoxydans, strain AMB1, and Methanoculleus bourgensis), when

639

incubated at 30°C, 38°C, and 46°C. The parameters investigated were within the ranges 0.05-

640

0.34 M NH4Cl, 30-46°C, and 0.05-0.4 M sodium acetate.

641

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